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猪和人表皮细胞单层培养中膜糖缀合物的合成与周转

Synthesis and turnover of membrane glycoconjugates in monolayer culture of pig and human epidermal cells.

作者信息

Davies H W, Trotter M D

出版信息

Br J Dermatol. 1981 Jun;104(6):649-58. doi: 10.1111/j.1365-2133.1981.tb00751.x.

Abstract

The regression and turnover of the surface glycoconjugates of trypsin-prepared pig and human cultured epidermal cells have been determined using the glycoprotein precursors N-acetyl-D-(I-3H) glucosamine (3H-NAG) and N-(3H)-acetyl-D-mannosamine (3H-NAM). Sialic acid assays have been performed on similar unlabelled cells. The major points which emerged from this study were: (1) Trypsin-damaged cell surfaces are rapidly repaired, probably by normal membrane turnover. There was a 12% regeneration of sialic acid within 2 h and total resynthesis occurred within 24 h. (2) The presence of an internal membrane system, part of which also demonstrates turnover, probably contributed to the speed of surface membrane repair. Some of the glycoprotein/sialic acid of this internal membrane system (30%) remains bound for a considerable length of time. (3) The membrane turnover maintains the cell in equilibrium so that total loss equals the synthesis of glycoprotein. (4) The equilibration of 3H-NAG or 3H-NAM uptake between 24 and 48 h is limited by the relative concentrations of glucose and labelled sugar in the medium at this time. (5) 3H-NAm was a more specific marker of glycoprotein than 2H-NAG. (6) The results for human epidermal cells closely matched those for pig epidermal cells, indicating that pig cells can be used as a model for human cells.

摘要

利用糖蛋白前体N-乙酰-D-(I-3H)葡萄糖胺(3H-NAG)和N-(3H)-乙酰-D-甘露糖胺(3H-NAM),测定了胰蛋白酶处理的猪和人培养表皮细胞表面糖缀合物的回归和周转情况。对类似的未标记细胞进行了唾液酸测定。这项研究得出的主要观点如下:(1)胰蛋白酶损伤的细胞表面可能通过正常的膜周转迅速修复。2小时内唾液酸再生12%,24小时内完全重新合成。(2)内膜系统的存在,其部分也表现出周转,可能有助于表面膜修复的速度。该内膜系统的一些糖蛋白/唾液酸(30%)会在相当长的时间内保持结合状态。(3)膜周转使细胞保持平衡,因此总损失等于糖蛋白的合成。(4)24至48小时之间3H-NAG或3H-NAM摄取的平衡受此时培养基中葡萄糖和标记糖相对浓度的限制。(5)3H-NAm是比3H-NAG更特异的糖蛋白标记物。(6)人表皮细胞的结果与猪表皮细胞的结果非常匹配,表明猪细胞可作为人细胞的模型。

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